Chemical composition of seeds of two okra cultivars - Journal of

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J. Agrlc.

~ o o dChem. 1083, 31, 1355-1358

These findings support the hypothesis that the principal cause for the observed vigor and higher yield in fresh weight of the tobacco plants that were treated with aldicarb is its effect on the carbohydrate (increase) and protein (decrease) content of the plant. Other things being equal, the higher concentration of water-soluble sugars in the treated plants may have developed a higher osmotic pressure that increases the absorption and/or retention of water in the plant tissue. This is reflected in the whole plant as an apparently higher yield and enhanced plant vigor. In a biological system, such as the tobacco plant, the presence of a bioactive compound like aldicarb in its tissue could result in complex phenomena of interactions. Investigations regarding such interactions are very complicated and the interpretation is difficult. Further research would be necessary to elucidate the mechanisms involved in such complex phenomena. Registry No. Aldicarb, 116-06-3;nicotine, 54-11-5; nitrate redudase, 9013-03-0;Fe, 7439-89-6;Mn, 7439-96-5;Zn,7440-66-6; K, 7440-09-7; Cu, 7440-50-8;Na, 7440-23-5.

LITERATURE CITED Allinson, D. W.; Peters, R. A. Agron. J. 1970, 62, 246. Chopra, S. L.; Sethi, R. K.; Sikka, V. K. Indian J. Agric. Chem.

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Heme, R. P. “A textbook of soil chemical analysis”;John Murray: London, 1971. Inman-Bamber,N. G.;Tainton, N. M. Roc.-Grassl. SOC.South Afr. 1972, 7, 130. IS0 (InternationalStandard Organization)“Tobacco and tobacco products”; ISO: Germany, 1972;Tech. Bull. ISO/DIS 2881. Jacobson, L. Plant Physiol. 1945, 20, 233. Jaiswal, P. S.; Saini, N. K.; Sharma, S. K. Plant Soil 1973, 38, 33.

Kalekenov, D. K. “Microelementy i estestvennaja Radioactivnost”; Pochvenij Rostovskogo Gosudarstvennogo Universiteta: Materialy Tretiego Mezhdunarodnogo Soveshchanija,1961; pp 152-155. Meyer, B. S.; Anderson, D. B.; Bohning, R. H. “Introductionto Plant Physiology”;Van Nostrand: London, 1960; pp 67,246. Nelson, M. J. Biol. Chem. 1944, 153, 375. Ries, S. K.; Chmiel, H.; Dilley, D. R.; Filner, P. Proc. Natl. Acad. Sci. U.S.A. 1967, 58, 526.

Ries, S. K.; Gast, A. Weeds 1965, 13, 272. Singh, B.; Vadhwa, 0. P.; Wu, M. T.; Salunkhe, D. K. J. Agric. Food Chem. 1972,20, 1256. Singh, B.; Wort, D. J. Plant Physiol. 1969, 44, 1321. Stewart, G. R.; Lee, J. A.; Orebamjo, T. 0. New Phytol. 1973,72, 539. Tso, T. C. “Physiology and Biochemistry of tobacco plants”; Dowden, Hutchinson, and Ross: Stroudsburg, PA, 1972a;p 36. TSO,T. C. “Physiology and Biochemistry of tobacco plants”; Dowden, Hutchinson, and Ross: Stroudsburg, PA, 1972b; p 42.

1974, 7, 7.

Coil, B. J.; Slattery, M. C. Plant Physiol. 1948, 23, 424. Croy, L. I. Ph.D. Thesis, University of Illinois, Urbana, IL, 1967. Deschreider, A. R.; Van Collie, L. “The trace metals in fresh vegetables”;Ministere Affaires Economy: Bruxelles, Belgium, 1952; Lab. Central Publ. 135, p 12. Eaton, S. V. Bot. Gaz. (Chicago)1952,114, 165. Finke, R. L.; Warner, R. L.; Muzik, T. J. Weed Sci. 1977,25, 18. Gaines, T. P. Ga., Agric. Exp. Stn., Res. Rep. 1971, No. 97. Hageman, R. H.; Flesher, D. Plant Physiol. 1960,35, 700.

Tsui, Cheng Am. J. Bot. 1948, 35, 172. Union Carbide Corp. “Technical information on Temik-10 G Aldicarb pesticide”;Union Carbide Corp.: New York, 1971. Vergara, B. S.; Miller, M.; Avelino, E. Agron. J. 1970, 62, 269. Wort, D. J.; Singh, B. Agron. J. 1970, 62, 57. Zsoldos, F. Plant Soil 1974, 41,41. Received for review March 19,1982. Revised manuscript received April 15, 1983. Accepted August 10, 1983.

Chemical Composition of Seeds of Two Okra Cultivars Hussain Al-Wandawi

Chemical compositions of the whole mature seeds of two okra varieties were investigated. The results of amino acid analyses indicated okra seed as a potential high-protein source which due to its high lysine level may serve as a supplement to cereal-based diets in which lysine is generally the first limiting amino acid. The most limiting amino acids in the Emerald variety were found to be valine (chemical score, 54.05), isoleucine (54.31), and threonine (60.0), while in the Ibtaira variety, tryptophan, isoleucine, and valine were the most limiting amino acids with chemical scores of 56.67, 57.41, and 67.03, respectively. The results of fatty acid analyses indicaed okra seed oil is akin to other high oleic acid oils and thus is of low essential fatty acid content. The most predominant elements in okra seed were found to be K, Na, Mg, and Ca. The elements Fe, Zn, Mn, and Ni were also present in abundant amounts. Gossypol was found only as traces, while Halphen-positive cyclopropenoid compounds were detected in an amount equal to 2.5 times less than that present in crude cotton oil.

In response to the present deficit and the predicted world shortage of foods, considerable research is being directed toward expanding present supplies and exploring new sources. Okra [Abelmoschus esculentus (L) Moench], appears to have potential as a high-protein crop when Food Science & Food Technology Division, Department of Agriculture & Biology, Nuclear Research Center, Baghdad, Iraq.

grown for its seed. Chemical and nutritional studies by Karakoltsidis and Constantinides (1975) on whole mature seeds of okra, Variety Emerald, have shown that the amino acid composition of okra was similar to that of soybeans and that the protein efficiency ratio (PER) was higher for okra. Martin et al. (1979) reported that a high-protein, high vegetable oil product can be prepared from okra seeds at the household level by using simple techniques. Savello et al. (1980) also reported on the nutritional composition of a seed meal prepared from an okra variety grown in 0 1983 American Chemical Society

1356 J. Agric. Food Chem., Vol. 31, No. 6, 1983

Puerto Rico. The present study compares the amino acids, fatty acids, gossypol, fiber, starch, and mineral compositions of one of Iraqi okra variety, namely, Ibtaira, which is known for its very high yield when grown for seeds with that of Emerald variety, since such a knowledge will be of interest in evaluating the nutritional value of this local variety. MATERIALS AND METHODS

Seed Sample. Seeds of both varieties were yield of plants grown under identical field conditions. Seed Flours. Seeds were visually sorted for uniform size, color, and maturity. For flour preparation, about 600 seeds wee ground to a fine powder in an electric mill. The powder thus obtained WBS used for all subsequent analyses. Amino Acid Analysis. A sample (500 mg) was hydrolyzed with 300 mL of glass-distilled 6 N HC1 a t reflux temperature (105 "C) under a fine stream of high-purity NZ. A trap, consisting of pyrogalol solution (Mondino and Bongiovanni, 1970), was used to free the Nzfrom any traces of Oz. The bubbling was maintained during the entire period of hydrolysis (22 h) and during the period required to cool the hydrolysate to room temperature. The hydrolysate thus obtained was filtered and evaporated to dryness on a rotary evaporator at 35-40 "C, and the residue was washed twice with a 2-mL portion of deionized distilled water, dissolved in 25 mL of citrate buffer (pH 2.2), kept overnight a t 4 "C, and filtered. The volume of the filtrate was adjusted to 25 mL. Finally 1 mL was transferred to a 5-mL volumetric flask and the volume was made up to the mark. A 0.1-mL portion was used for amino acid analysis using a Beckman Model 120C amino acid analyzer following the procedure described by the manufacturer. Tryptophan. Due to its destruction during acid hydrolysis, tryptophan was determined by hot-alkaline hydrolysis. A sample (100 mg) was mixed with 3 g of Ba(0H),.8Hz0 followed by addition of 6 mL of distilled water, and mixed thoroughly. Hydrolysis and quantitation were carried out following the method reported by Kehayoglou and Manoussopouls (1977). Oil Extraction and Fatty Acid Analysis. Lipids were obtained by extraction of okra seed flour with redistilled hexane (1:20 w/v) in a Soxhlet extractor for 4 h. After extraction, solvent was removed by using a rotary evaporator and the oil kept in dark under high-purity Nz gas until required for analysis. Fatty Acid Analysis. About 25 mg of total lipids was transesterified by using methanol-HC1 reagent (procedure A). In procedure B, about 150 mg of lipids was saponified by refluxing with 5 mL of 0.5 N methanolic NaOH (in the dark and under a fine stream of high-purity nitrogen gas) for 5 min. Then esterification was achieved by adding 5 mL of BF,-methanol complex reagent and the mixture was refluxed for 4 min. The fatty acid esters were then recovered by adding 5 mL of 2% aqueous NaCl solution and 10 mL of peroxide free diethyl ether. The fatty acid esters prepared by each of the above methods were determined on a Packard Model 419 gas chromatograph using an FID and a glass column (20.1 X 2 mm) packed with 3% SE-30 on Diatomite C (100-120 mesh). Detector and injector temperature was 120 "C and oven temperature 100-220 "C, 4 "C/min. Fatty acid esters were identified by comparing their retention times with those of known references, and the individual fatty acids were quantified by the method of triangulation. Gossypol. Total gossypol was determined by using a procedure developed by Pons et al. (1958), while free gossypol was determined by using two different procedures

AI- Wandawi

Table I. Chemical Composition of Okra Seeds %' (dry weight basis) for variety

protein ( N X 6.25) moisture ash lipids crude fiber starchb total carbohydrateC

Emerald

Ibtaira

21.82" i1.33d 6.96y * 0.38 4.33y i 0.02 14.70y i 0.57 27.3OY i0.28 4.75y i0.14 24.89 c 0.65

17.66y ? 0.22d 6.84x i 0.16 4.62x i 0.04 16.65x t 0.78 27.20x t 0.14 5.00' ? 0.28 27.14x i 0.90

a Mean * SD. Values expressed as percent of defatted and sugar-free flour. Total carbohydrate is determined as 100 - (moisture t protein t lipids t crude fiber t ash). Means followed by same letter on a horizontal line are significantly different according to an L.S.D.test (P= 0.05).

(Storherr and Helley, 1954; S c h r a " and Benedict, 1958). Cyclopropenoid compounds were determined by using the Halpen test (Association of Official Analytical Chemists, 1975). Crude Fiber. Crude fiber was determined by using the fibertec system Model 1010 Heat Extract, Tecator (Sweden) following the procedure described by the manufacturer. Starch. One gram of defatted flour was extracted with 100 mL of 95% EtOH in a Soxhlet extractor for 4 h. The sugar-free residue thus obtained was dried overnight at 45-50 "C in an vacuum oven; then 100-mg samples were refluxed with 500 mL of 0.4 N H2S04for 4 h, followed by cooling to room temperature and filtering. The filtrate was up to 1 L. A portion (200 mL) was adjusted to pH 7.0 by addition of few milliliters of 50% KOH and left to stand in an ice bath for 15 min prior to centrifugation a t 10000 rpm for 15 min at (2 "C). The supernatant was decanted and reserved, while the precipitate was reextracted with 100-mL of distilled water. The supernatants were pooled and made up to a known volume. A 50-mL portion was evaporated a t 45-50 "C. The residue was dissolved in 2 mL of distilled water, the flask was rinsed with another 2-mL portion of distilled water, and the final volume was adjusted to 5 mL. Starch was determined as glucose by using anthrone reagent. Standard starch (potato starch) was treated similarly, and the resulting glucose showed excellent recovery (98.5-99.0 %). Minerals. The elements Ca, Mg, K, and Na were determined by using a 503 Perkin-Elmer atomic absorption spectrometer following the method described by the manufacturer. The elements Cu, Cr, Fe, Mn, Ni, Rb, Sr, and Zn were determined by the secondary absorption correction method (Jenkins, 1974) using a Philips 1140/00 X-ray spectrometer. RESULTS

The results of chemical analyses of the major constituents of the whole mature seeds of a local okra cultivar, "Ibtaira", are presented and compared to the "Emerald" variety (Table I). The cultivars are similar in their crude fiber, ash, starch, total carbohydrate, gossypol, and moisture contents. Protein level, on the other hand, is slightly higher in Emerald, while Ibtaira shows a slightly higher lipid level. The results of the amino acid contents of the seeds of both cultivars are presented in Table 11. The results reveal that with the exception of glutamic acid and arginine, which show higher levels in Emerald, and alanine, which is higher in Ibtaira, all other amino acids in both cultivars are either similar or slightly higher in Emerald. Fatty acid compositions of okra seed lipids are

J. Agric. FoodChem., Vol. 31, No. 6,1983

Chemical Composition of Seeds of Two Okra Cultivars

Table 11. Amino Acid Composition (Grams per 16 Grams of N ) of Okra Seeds variety amino acid LY s His Arg TrP Asp Th Ser Glu Pro GlY Ala CYS Val Met Ile Leu TYr Phe

Emerald 7.24y i 1.78y i 11.04y * 0.96y t 11.82y t 3.02y * 5.25y i 22.08y i 3.83y i 6.13y i 5.51Y i 2.45y t 4.OOy ? 1.66y i 3.15Y 2 6.68y 2 3.6gY i 4.28y i

O.Ogapb 0.17 0.10 0.11 0.48 0.10 0.30 0.82 0.28 0.21 0.04 0.14 0.04 0.13 0.14 0.16 0.17 0.21

Ibtaira 8.9OYt 1.83x * 10.16y i 0.85x t 13.17" t 3-49" * 6.35x i 20.74" i 4.18" i 6.66xi 6.66y i 2.53x i 4.95y i 1.85x i 3.32x i 7.03x i 3.83"+ 3.93x i

0.28a,b 0.13 0.23 0.03 0.27 0.27 0.21 0.51 0.26 0.24 0.34 0.07 0.16 0.13 0.16 0.14 0.20 0.13

a Means i SD. Means followed by same letter o n a horizontal line are significantly different according to an L.S.D. test (P= 0.05).

shown in Table 111. Oleic acid, palmitic acid, and stearic acid are the major fatty acid constituents in both cultivars. In the Emerald variety, palmitic and stearic acid levels are in good agreement with data reported by Karakoltsidis and Constantinides (1975), while oleic acid is found in much higher levels in comparison with data reported by the same authors. Comparison of chemical score values of essential amino acids of okra seeds with those of wheat and soybean is shown in Table IV. Okra seed seems to be rich of lysine; thus, the chemical score for lysine was found to be close to that of soybean. Elemental compositions of the seeds of both varieties are shown in Table V. The elements K, Na, Mg, and Ca are the major elemental constituents, while Fe, Mn, Zn, and Sr are present in the range of 2-10 mg/100 g of defatted seed flour. Other elements are found in the range of